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Conformationally restricted nucleotides as a probe of structure-function relationships in RNA.

机译:构象受限的核苷酸作为RNA中结构与功能关系的探针。

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摘要

We introduce the use of commercially available locked nucleic acids (LNAs) as a functional probe in RNA. LNA nucleotides contain a covalent linkage that restricts the pseudorotation phase of the ribose to C3'-endo (A-form). Introduction of an LNA at a single site thus allows the role of ribose structure and dynamics in RNA function to be assessed. We apply LNA probing at multiple sites to analyze self-cleavage in the lead-dependent ribozyme (leadzyme), thermodynamic stability in the UUCG tetraloop, and the kinetics of recognition of U1A protein by U1 snRNA hairpin II. In the leadzyme, locking a single guanosine residue into the C3'-endo pucker increases the catalytic rate by a factor of 20, despite the fact that X-ray crystallographic and NMR structures of the leadzyme ground state reported a C2'-endo conformation at this site. These results strongly suggest that a conformational change at this position is critical for catalytic function. Functional insights obtained in all three systems demonstrate the highly general applicability of LNA probing in analysis of the role of ribose orientation in RNA structure, dynamics, and function.
机译:我们介绍了使用市售的锁定核酸(LNA)作为RNA中的功能探针。 LNA核苷酸包含共价键,该键将核糖的假旋转阶段限制为C3'-endo(A形式)。因此,在单个位点引入LNA可以评估核糖结构的作用和RNA功能的动力学。我们在多个位置应用LNA探测,以分析铅依赖性核酶(铅酶)中的自我切割,UUCG四环中的热力学稳定性以及U1 snRNA发夹II对U1A蛋白的识别动力学。在铅酶中,将单个鸟苷残基锁定在C3'-endo褶皱中可将催化速率提高20倍,尽管事实上铅酶基态的X射线晶体学和NMR结构表明C3'-endo构象在这个网站。这些结果强烈表明,该位置的构象变化对于催化功能至关重要。在这三个系统中获得的功能见解证明了LNA探测在核糖方向在RNA结构,动力学和功能中的作用分析中的高度通用性。

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